Abstract

Thermus thermophilus MutS, a thermostable mismatch-recognizing protein, is utilized in PCR to suppress nonspecific amplification by preventing synthesis from mismatched primers. T. thermophilus RecA also decreases nonspecific amplification by promoting proper hybridization between the primer and template. We observed that MutS and RecA function under the same reaction conditions and that MutS and RecA do not preclude each other. Furthermore, there were some DNA sequences for which only one of the 2 proteins effectively suppressed nonspecific amplification. The simultaneous use of MutS and RecA is a more attractive error-suppressing technique than the use of either of the 2 proteins alone.

1. Introduction

PCR-based technologies are essential for a wide range of biosciences, ranging from basic life sciences to medical diagnoses [13]. The efficiency and reliability of those technologies are often decreased by nonspecific amplifications resulting from mishybridization of primers. Recently, we developed a technique to suppress nonspecific amplification by adding a thermostable mismatch-recognizing protein Thermus thermophilus MutS (ttMutS) in PCR mixture [4]. MutS is a DNA mismatch repair protein, which recognizes a variety of DNA mismatches such as base-base mismatches and base insertion loops [5, 6]. MutS is thought to bind tightly to the mismatched bases that are generated by mishybridization between primer and template to block the association of a DNA polymerase. Before we established the MutS-based error-suppressing technique, it had been reported that T. thermophilus RecA (ttRecA) protein can be used to decrease nonspecific amplification during PCR, which drastically enhances the accuracy of multiplex PCR [7]. RecA is known to be a key enzyme in homologous recombination of DNA molecules, which catalyzes pairing of 2 homologous sequences [8]. The ttRecA protein enhances the proper pairing between the primer and template to suppress nonspecific amplification. Thus, the mechanisms by which ttMutS and ttRecA suppress nonspecific amplification are quite different. In this study, we investigated the difference in the effects and properties of ttMutS and ttRecA in order to evaluate the possibility of simultaneous use of both proteins.

2. Materials and Methods

2.1. Overexpression and Purification of Proteins

Thermus thermophilus MutS (ttMutS) was prepared as previously described [4]. A DNA fragment-expressing T. thermophilus RecA (ttRecA) was generated by PCR using the T. thermophilus HB8 genomic DNA as a template. The following primer pairs were used for amplification of the fragment: 5′-ATATCATATGGACGAGAGCAAGCGCAAGGC-3′ and 5′-ATATGGATCCTTATTACTCCCCCTCGTCCTCGCCC-3′. The forward and reverse primers contained NdeI and BamHI restriction sites, respectively (underlined). The amplified fragment was ligated into the NdeI and BamHI sites of pET-11a (Novagen, Madison, WI, USA) to obtain pET-11a/T. thermophilus recA. Sequence analysis revealed that the construction was error-free. E. coli BL21 (DE3) was transformed with pET-11a/T. thermophilus recA and then grown at 37°C in 1.5 liters of YT medium containing 50  g/mL of ampicillin. When the density of cultures reached 2.9 × 108 cells/mL, isopropyl -D-thiogalactopyranoside was added to 100  M. The cells were grown at 37°C for 3 h after induction and harvested by centrifugation. The cells were lysed by sonication in 50 mM Tris-HCl (pH 7.5) containing 100 mM NaCl and 1.5 M KCl and then heated to 60°C for 60 min. After centrifugation at 48,000 ×g for 20 min, the supernatant was isolated, and ammonium sulfate was added to a final concentration of 1.5 M. The solution was loaded onto a TOYOPEARL-Phenyl column (12 mL, TOSOH, Tokyo, Japan) preequilibrated with 50 mM Tris-HCl (pH 8.0) containing 1.5 M ammonium sulfate. The column was washed with the same buffer and then eluted with 1.5–0 M ammonium sulfate gradient in the same buffer. The fraction containing ttRecA was detected by SDS-PAGE and dialyzed against 50 mM Tris-HCl (pH 8.0). The solution was loaded onto a TOYOPEARL-DEAE column (12 mL, TOSOH) preequilibrated with 50 mM Tris-HCl (pH 8.0). The column was washed with the same buffer and then eluted with 0–1.5 M KCl gradient in 50 mM Tris-HCl (pH 8.0).

2.2. PCR Using ttRecA and ttMutS Proteins

The 5′-terminal 423-bp region of the ttha1806 gene was amplified using the primers 5′-GAGACCACCCGTAGGCGGCT-3′ and 5′-CTTAAGGGGCCTCGCGCTCT-3′; a 1,278-bp region of the ttha1548 gene was amplified using 5′-GAGGAGGTGCTCTACGTGGGCAAGGCC-3′ and 5′-GGGAAGGTCCTTGAGGCTTCCCGTGTAGC-3′; a 611-bp region of the ttha0122 gene was amplified using 5′-ATGTTCCTGAGGATAGACCGCC-3′ and 5′-ATCTCCACCCCGGTGAGGC-3′; and a 466-bp region of the ttha1300 gene was amplified using 5′-ATGCCCGCCATGGAAGTGG-3′ and 5′-TGAGCGCCTTCAGGGCCT-3′. The primers were synthesized by BEX Co. (Tokyo, Japan). The reactions were performed in 1 × Takara GC I buffer (Takara, Shiga, Japan) containing 0.06 units/ L Takara LA Taq (Takara), 5 ng/ L T. thermophilus HB8 genomic DNA, 400 nM primers, 100  M CoCl2, and 400  M dATP, dTTP, dCTP, and dGTP (Takara) in the presence of various concentrations of ttRecA and ttMutS. Thirty PCR cycles were run using ASTEC OC707 (ASTEC, Tokyo, Japan): denaturation step at 95°C for 1 min, annealing at 58°C for 1 min, and extension at 70°C for 2 min for amplification of the ttha1806 gene; and denaturation step at 95°C for 1 min, annealing at 50°C for 1 min, and extension at 70°C for 2 min for amplification of the ttha0122, ttha1300, and ttha1548 genes. A 10  L reaction solution was mixed with 1  L of loading buffer (50% [v/v] glycerol, 0.9% [w/v] SDS, and 0.05% [w/v] bromophenol blue) and electrophoresed on a 1.5% agarose gel in 1 × TBE buffer. The gel was stained with ethidium bromide, and the products were visualized under ultraviolet light at 254 nm. The relative amounts of the amplified DNA products were quantified using the ImageJ software [10].

3. Results and Discussion

As has been previously described, RecA catalyzes the homologous pairing of DNA molecules in an ATP-dependent manner [1113], and ttRecA requires ATP for the error-suppressing effect during PCR [7]. On the other hand, ATP is not essential for the error-suppressing effect of ttMutS during PCR [4]. However, it is known that MutS has a Walker’s A-type ATPase motif [14, 15] and that the conformation and function of MutS are greatly affected by the binding and hydrolysis of ATP. Binding of ATP triggers the formation of sliding-clamp mode of MutS, and enhances the dissociation of MutS from a mismatch [10, 16]. Therefore, we examined whether or not ATP interferes with the error-suppressing effect of MutS during PCR. The 423-base pair (bp) region of the ttha1806 gene was amplified by Takara LA Taq using T. thermophilus HB8 genomic DNA as the template. Without ttMutS and ttRecA, 1000- to 5000-bp DNA fragments were amplified nonspecifically (Figure 1(c)). ttMutS showed a significant suppressing effect on the nonspecific amplifications in the presence of 0 to 0.4 mM ATP (Figure 1(c)). The previous reports described that 0.4 mM ATP is enough to ensure the maximum effect of ttRecA [7], which was also supported by our results (Figure 1(c)). It also should be noted that 0.4 mM ATP did not influence the specificity of PCR amplification (Figure 1(c), left panel). Thus, ttMutS and ttRecA function under the same reaction conditions. We also demonstrated that 0.4  M ttRecA and 0.8  M ttMutS were suitable for suppressing the nonspecific amplifications during PCR, with a wide range of template concentrations (0.9 to 24 ng/ L) (Figure 1(d)). Since ttMutS and ttRecA are not stable at the temperature over 90°C, the error-suppressing effect may be improved by supplementing the reaction with additional proteins at the middle of the PCR cycle. However, as shown in our data, we were able to obtain satisfactory effect without the supplementation when we use 0.4  M ttRecA and 0.8  M ttMutS. The supplementation of the additional proteins may be required when we cannot obtain enough effect under these conditions.

To determine whether ttRecA and ttMutS preclude the effect of each other, a 611-bp region of the ttha0122 gene was amplified by Takara LA Taq using T. thermophilus HB8 genomic DNA as a template. In the absence of ttRecA and ttMutS, relatively weak amplification of the target sequence and the nonspecific amplification of 1000- to 1500-bp were observed (Figure 2(a)). Both ttRecA and ttMutS enhanced the amplification of the desired fragment and suppressed the nonspecific amplification (Figure 2(a)). The error-suppressing effect was retained when both ttRecA and ttMutS were present (Figure 2(a)). The same result was also obtained when the 423-bp region of the ttha1806 gene was amplified in the presence of ttRecA and aqMutS (Figure 2(b)). These findings suggest that ttRecA and ttMutS can be used simultaneously without any interfering effects.

In order to evaluate the validity of the simultaneous use of ttRecA and ttMutS, we investigated the difference in the specificities of ttRecA and ttMutS towards the sequences to be amplified. If their error-suppressing effects show different specificities for the target sequences, simultaneous use would cover a wider range of sequences than the single use of ttRecA or ttMutS would. As shown in Figure 2(c), nonspecific amplification upon the amplification of a 466-bp region of the ttha1300 gene was effectively suppressed by ttRecA but not by ttMutS. In contrast, ttMutS showed a strong error-suppressing effect on the amplification of a 1,278-bp region of the ttha1548 gene, whereas ttRecA did not (Figure 2(d)). These results clearly indicate that ttRecA and ttMutS have distinct specificities against the target sequences. This is expected because ttRecA and ttMutS suppress nonspecific amplification in different ways.

4. Conclusions

In this study, we clarified that ttMutS and ttRecA do not preclude each other and there are some sequences for which only one of the 2 proteins efficiently suppresses nonspecific amplification. Our results in this study suggest that simultaneous use of ttMutS and ttRecA is better than the use of either ttMutS or ttRecA alone.

Conflict of Interests

The publication of this paper may affect the value of the patent for the methodology described in our previously published paper [6].

Acknowledgments

The authors express great thanks to Dr. Yoshitaka Bessho for his valuable discussions, to Dr. Ryoji Masui (Osaka University) and Tomofumi Sakai (Osaka University) for overexpression and purification of ttRecA, and to Kayoko Matsumoto (RIKEN SPring-8 Center) for her excellent help in overexpression of ttMutS. This work was supported by Management Expenses Grants from the government to RIKEN.